Potato cultivar Y9

ABSTRACT

A potato cultivar designated Y9 is disclosed. The invention relates to the tubers of potato cultivar Y9, to the seeds of potato cultivar Y9, to the plants of potato cultivar Y9, to the plant parts of potato cultivar Y9, to food products produced from potato cultivar Y9, and to methods for producing a potato plant produced by crossing potato cultivar Y9 with itself or with another potato variety. The invention also relates to methods for producing a potato plant containing in its genetic material one or more transgenes and to the transgenic potato plants and plant parts produced by those methods. This invention also relates to potato cultivars or breeding cultivars and plant parts derived from potato variety Y9, to methods for producing other potato cultivars, lines or plant parts derived from potato cultivar Y9 and to the potato plants, varieties, and their parts derived from use of those methods. The invention further relates to hybrid potato tubers, seeds, plants and plant parts produced by crossing potato cultivar Y9 with another potato cultivar.

CROSS-REFERENCE TO RELATED APPLICATIONS

The present application claims the benefit of priority to U.S. Provisional Application No. 62/239,068, filed on Oct. 8, 2015, and U.S. Provisional Application No. 62/256,940, filed on Nov. 18, 2015, the entire contents of each of which are hereby incorporated by reference in their entirety for all purposes.

FIELD

The present disclosure relates to a novel potato cultivar designated Y9 and to the tubers, plants, plant parts, tissue culture, and seeds produced by that potato variety. The disclosure further relates to food products produced from potato cultivar Y9, such as French fries, potato chips, dehydrated potato material, potato flakes, and potato granules.

BACKGROUND

The potato is the world's fourth most important food crop and by far the most important vegetable. Potatoes are currently grown commercially in nearly every state of the United States. Annual potato production exceeds 18 million tons in the United States and 300 million tons worldwide. The popularity of the potato derives mainly from its versatility and nutritional value. Potatoes can be used fresh, frozen or dried, or can be processed into flour, starch or alcohol. They contain complex carbohydrates and are rich in calcium, niacin and vitamin C.

The quality of potatoes in the food industry is affected by two critical factors: (1) potatoes contain large amounts of asparagine, a non-essential free amino acid that is rapidly oxidized to form acrylamide, a carcinogenic product, upon frying or baking; and (2) potatoes are highly susceptible to enzymatic browning and discoloration, an undesirable event which happens when polyphenol oxidase leaks out from the damaged plastids of bruised potatoes. In the cytoplasm, the enzyme oxidizes phenols, which then rapidly polymerize to produce dark pigments. Tubers contain large amounts of phosphorylated starch, some of which is degraded during storage to produce glucose and fructose. These reducing sugars react with amino acids to form Maillard products including acrylamide when heated at temperatures above 120° C. Two enzymes involved in starch phosphorylation are water dikinase R1 and phosphorylase-L (R1 and PhL). Browning is also triggered non-enzymatically as a consequence of the partial degradation of starch into glucose and fructose.

Many potato cultivars are susceptible to late blight, a devastating disease caused by the fungus-like oomycete pathogen Phytophthora infestans. Late blight of potato is identified by black/brown lesions on leaves and stems that may expand rapidly and become necrotic. Severe late blight epidemics occur when P. infestans grows and reproduces rapidly on the host crop.

Thus, there is a need to develop potato varieties with reduced levels of toxic compounds and increased resistance to disease, but without the use of unknown or foreign nucleic acids. The present disclosure satisfies this need.

The foregoing examples of the related art and limitations related therewith are intended to be illustrative and not exclusive. Other limitations of the related art will become apparent to those of skill in the art upon a reading of the specification.

SUMMARY OF THE DISCLOSURE

There is thus a need in the art for potato plant varieties that produce tubers with low acrylamide content, increased black spot bruise tolerance, lowered reducing sugars, and increased resistance to late blight.

The following embodiments and aspects thereof are described in conjunction with systems, tools and methods which are meant to be exemplary, not limiting in scope. In various embodiments, one or more of the above-described problems have been reduced or eliminated, while other embodiments are directed to other improvements.

To this end, the present invention provides novel potato variety Y9 transformed with nucleic acid sequences that are native to the potato plant genome and does not contain foreign DNA, Agrobacterium DNA, viral markers or vector backbone sequences. Rather, the DNA inserted into the genome of the potato variety Y9 is a non-coding polynucleotide native to potato or native to wild potato, a potato sexually-compatible plant, that silences genes involved in the expression of black spot bruises, asparagine accumulation and senescence sweetening.

Thus, in one embodiment, the present invention provides a plant vector, referred to as pSIM1278, that comprises a first silencing cassette containing two copies of a DNA segment comprising, in anti-sense orientation, a fragment of the asparagine synthetase-1 gene (fAsn1) and the 3′-untranslated sequence of the polyphenol oxidase-5 gene; and a second silencing cassette containing two copies of a DNA segment comprising, in anti-sense orientation, a fragment of the potato phosphorylase-L (pPhL) gene and a fragment of the potato R1 gene. The pSIM1278 vector comprises a 9,512 bp backbone region that supports maintenance of the plant DNA prior to plant transformation and is not transferred into plant cells upon transformation of the plant cells, and a 10,148 bp DNA insert region comprising native DNA that is stably integrated into the genome of the plant cells upon transformation.

In another embodiment, the present invention provides a second plant vector, referred to as pSIM1678, which comprises the Rpi-vnt1 expression cassette and a silencing cassette for the plant vacuolar invertase gene, VInv. The Rpi-vnt1 gene cassette consists of the VNT1 protein coding region regulated by its native promoter and terminator sequences to confer broad resistance to late blight, whereas the silencing cassette consists of an inverted repeat of sequence from the potato VInv gene flanked by opposing plant promoters, pGbss and pAgp. The pSIM1678 vector comprises a 9,512 bp backbone region that supports maintenance of the plant DNA prior to plant transformation and is not transferred into plant cells upon transformation of the plant cells, and a 9,090 bp DNA insert region comprising native DNA that is stably integrated into the genome of the plant cells upon transformation.

In a different embodiment, the invention provides a plant cell transformed with one or both of the plant vectors of the invention. In a further embodiment, the invention provides a potato plant variety comprising one or more cells transformed with the vectors of the invention. In one aspect of the invention, the potato plant variety expresses at least one of the two silencing cassettes of the vector pSIM1278 and expresses the silencing cassette of the vector pSIM1678, and expression of the silencing cassettes results in the down-regulation of the asparagine synthetase-1 gene, the polyphenol oxidase-5 gene and the vacuolar invertase gene in the tubers of the plant. In a preferred aspect of the invention, the tubers of the potato plant variety expressing at least one silencing cassette display two or more desirable traits that are not present in the tubers of untransformed plants of the same variety. In the most preferred aspect of the invention, the two or more desirable traits are selected from the group consisting of low asparagine accumulation, reduced black-spot bruising, reduced heat-induced acrylamide formation and reduced accumulation of reducing sugars during storage.

In a different aspect of the invention, the potato plant variety expresses both silencing cassettes of the plant DNA vector pSIM1278, and expresses the silencing cassette of the vector pSIM1678, and expression of the silencing cassettes results in the down-regulation of the asparagine synthetase-1 gene, the polyphenol oxidase-5 gene, the phosphorylase-L gene, the dikinase R1 gene and the vacuolar invertase gene in the tubers of the potato plant variety. In a preferred aspect of the invention, the tubers of the potato plant variety expressing two silencing cassettes of the plant DNA vector pSIM1278 and expressing the silencing cassette of the vector pSIM1678 display two or more desirable traits that are not present in the tubers of untransformed plants of the same variety. In a preferred embodiment, the two or more desirable traits are selected from the group consisting of low asparagine accumulation, reduced black-spot bruising, reduced accumulation of reducing sugars during storage and reduced heat-induced acrylamide formation. In one aspect of the invention, the potato plant variety expressing the two silencing cassettes of the plant DNA vector pSIM1278 and the silencing cassette of the plant DNA vector pSIM1678 is the Atlantic Y9 variety.

In another aspect of the invention, the potato plant variety Y9 of the present invention expresses the late blight resistance gene (Rpi-vnt1) of the plant DNA vector pSIM1678. In a further aspect of the present invention, the potato plant variety Y9 of the present invention has increased resistance to late blight infection.

Thus, according to the invention, there is provided a new potato cultivar of the genus and species Solanum tuberosum L. designated Y9. This invention thus relates to potato cultivar Y9, to the tubers of potato cultivar Y9, to the plants of potato cultivar Y9, to the seeds of potato cultivar Y9, to the food products produced from potato cultivar Y9, and to methods for producing a potato plant produced by selfing potato cultivar Y9 or by crossing potato cultivar Y9 with another potato cultivar, and the creation of variants by mutagenesis or transformation of potato cultivar Y9.

Thus, any such methods using the cultivar Y9 are embodiments of this invention: selfing, backcrosses, hybrid production, crosses to populations, and the like. All plants produced using potato cultivar Y9 as at least one parent are within the scope of this invention. Advantageously, the potato cultivar could be used in crosses with other, different, potato plants to produce first generation (F₁) potato hybrid tubers, seeds and plants with superior characteristics.

In another embodiment, the present invention provides for single or multiple gene converted plants of potato cultivar Y9. In one embodiment, the transferred gene(s) may be a dominant or recessive allele(s). In some embodiments, the transferred gene(s) will confer such traits as herbicide resistance, insect resistance, resistance for bacterial, fungal, or viral disease, male fertility, male sterility, enhanced nutritional quality, uniformity, and increase in concentration of starch and other carbohydrates, decrease in tendency to bruise and decrease in the rate of conversion of starch to sugars. The gene(s) may be a naturally occurring potato gene or a transgene introduced through genetic engineering techniques, backcrossing or mutation.

In another embodiment, the present invention provides regenerable cells for use in tissue culture of potato cultivar Y9. In one embodiment, the tissue culture will be capable of regenerating plants having all the physiological and morphological characteristics of the foregoing potato plant, and of regenerating plants having substantially the same genotype as the foregoing potato plant. In some embodiments, the regenerable cells in such tissue cultures will be embryos, protoplasts, meristematic cells, callus, pollen, leaves, anthers, pistils, cotyledons, hypocotyl, roots, root tips, flowers, seeds, petioles, tubers, eyes or stems. Still further, the present invention provides potato plants regenerated from tissue cultures of the invention.

In a further embodiment, the invention provides a food product made from a tuber of potato plant variety Atlantic Y9. Preferably, the food product is a heat-treated product. Even more preferably, the food product is a fresh whole potato, French fry, potato chip, dehydrated potato material, potato flakes, or potato granules.

In addition to the exemplary aspects and embodiments described above, further aspects and embodiments will become apparent by study of the following descriptions.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 depicts the pSIM1278 transformation vector. The vector backbone region, on the left, is 9,512 bp long, as it starts at position 10,149 bp and ends at position 19,660 bp. The backbone DNA consists mainly of bacterial DNA which provides support maintenance of the DNA insert prior to plant transformation. The DNA insert region (right side), including flanking Border sequences, is 10,148 bp long (from 1 bp to 10,148 bp). The DNA insert was stably integrated into the potato genome upon transformation.

FIG. 2 provides a schematic representation of the silencing cassettes in the DNA insert inserted in the pSIM1278 transformation vector. Each silencing cassette contains two copies of two gene fragments separated by a spacer. Two copies of a DNA segment comprising fragments of four targeted genes, namely Asn-1, Ppo-5, Phl and R1, were inserted as inverted repeats between two convergent promoters, indicated as Pro, that are predominantly active in tubers. Plants containing the resulting silencing cassette produce a diverse and unpolyadenylated array of RNA molecules in tubers that dynamically and vigorously silence the intended target genes. The size of the RNA molecules was generally smaller than the distance between the two promoters employed because convergent transcription results in collisional transcription.

FIG. 3 depicts the pSIM1678 transformation vector of the present invention. The vector backbone region, on the left, is 9,512 bp long, as it starts at position 9,091 bp and ends at position 18,602 bp. The backbone DNA consists mainly of bacterial DNA which provides support maintenance of the DNA insert prior to plant transformation. The DNA insert region (right side), including flanking Border sequences, is 9,090 bp long (from 1 bp to 9,090 bp). The DNA insert consists of native DNA only and was stably integrated into the potato genome upon transformation.

FIG. 4 provides a schematic representation of the silencing cassettes in the DNA insert inserted in the pSIM1278 transformation vector (upper construct) and the silencing cassette in the DNA insert inserted in the pSIM1678 transformation vector (lower construct)

FIG. 5 illustrates the process for constructing plasmid pSIM1278, utilizing the DNA sequences as described in Table 1 and Table 2. The starting vector, pCAMBIA1301, contains the origins of replications in the final pSIM1278 backbone.

FIG. 6 illustrates the construction of T-DNA expression cassettes in pSIM1278. Fusion PCR was used to amplify elements 1A (pAgp—1st copy), 1B (pAgp—2nd copy), 2 (Asn1, Ppo5), 3 (Ppo5, Asn1), 4 (pGbss—1st copy) and 7 (Spacer1, Ppo5, Asn1). Elements 5 (PhL, R1) and 6 (Spacer2, R1, PhL, pGbss) were synthesized by the Blue Heron Biotechnology, Inc. (Bothell, Wash.) based on the sequence from the potato genome. Elements 8, 9, and 10 were generated by ligating building blocks shown in the figure. In the end, three fragments, 10, 11 and 6 were created to span the desired expression cassette. These three fragments were ligated and inserted into the KpnI-SacI restriction sites shown in FIG. 5 to generate pSIM1278.

FIG. 7 illustrates the process for constructing plasmid pSIM1678, utilizing the DNA sequences as described in Table 3 and Table 4. The starting vector, pSIM1278, contains the final pSIM1678 backbone.

DETAILED DESCRIPTION Definitions

In the description and tables which follow, a number of terms are used. In order to provide a clear and consistent understanding of the specification and claims, including the scope to be given such terms, the following definitions are provided.

The term “a” or “an” refers to one or more of that entity; for example, “a primer” refers to one or more primers or at least one primer. As such, the terms “a” (or “an”), “one or more” and “at least one” are used interchangeably herein. In addition, reference to “an element” by the indefinite article “a” or “an” does not exclude the possibility that more than one of the elements is present, unless the context clearly requires that there is one and only one of the elements.

Allele. An allele is any of one or more alternative forms of a gene which relate to one trait or characteristic. In a diploid cell or organism, the two alleles of a given gene occupy corresponding loci on a pair of homologous chromosomes.

Amino acid sequence. As used herein, includes an oligopeptide, peptide, polypeptide, or protein and fragments thereof that are isolated from, native to, or naturally occurring in a plant, or are synthetically made but comprise the nucleic acid sequence of the endogenous counterpart.

Artificially manipulated. as used herein, “artificially manipulated” means to move, arrange, operate or control by the hands or by mechanical means or recombinant means, such as by genetic engineering techniques, a plant or plant cell, so as to produce a plant or plant cell that has a different biological, biochemical, morphological, or physiological phenotype and/or genotype in comparison to unmanipulated, naturally-occurring counterpart.

Asexual propagation. Producing progeny by generating an entire plant from leaf cuttings, stem cuttings, root cuttings, tuber eyes, stolons, single plant cells protoplasts, callus and the like, that does not involve fusion of gametes.

Backbone. Nucleic acid sequence of a binary vector that excludes the DNA insert sequence intended for transfer.

Backcrossing. Backcrossing is a process in which a breeder repeatedly crosses hybrid progeny back to one of the parents, for example, a first generation hybrid F₁ with one of the parental genotypes of the F₁ hybrid.

Bacterial Ring Rot. Bacterial ring rot is a disease caused by the bacterium Clavibacter michiganense ssp. Bacterial ring rot derives its name from a characteristic breakdown of the vascular ring within the tuber. This ring often appears as a creamy-yellow to light-brown, cheesy rot. On the outer surface of the potato, severely diseased tubers may show slightly sunken, dry and cracked areas. Symptoms of bacterial ring rot in the vascular tissue of infected tubers can be less obvious than described above, appearing as only a broken, sporadically appearing dark line or as a continuous, yellowish discoloration.

Black spot bruise. Black spots found in bruised tuber tissue are a result of a pigment called melanin that is produced following the injury of cells and gives tissue a brown, gray or black appearance. Melanin is formed when phenol substrates and an appropriate enzyme come in contact with each other as a result of cellular damage. The damage does not require broken cells. However, mixing of the substrate and enzyme must occur, usually when the tissue is impacted. Black spots occur primarily in the perimedullary tissue just beneath the vascular ring, but may be large enough to include a portion of the cortical tissue.

Border-like sequences. A “border-like” sequence is isolated from the selected plant species that is to be modified, or from a plant that is sexually-compatible with the plant species to be modified, and functions like the border sequences of Agrobacterium. That is, a border-like sequence of the present invention promotes and facilitates the integration of a polynucleotide to which it is linked. A DNA insert of the present invention preferably contains border-like sequences. A border-like sequence of a DNA insert is between 5-100 bp in length, 10-80 bp in length, 15-75 bp in length, 15-60 bp in length, 15-50 bp in length, 15-40 bp in length, 15-30 bp in length, 16-30 bp in length, 20-30 bp in length, 21-30 bp in length, 22-30 bp in length, 23-30 bp in length, 24-30 bp in length, 25-30 bp in length, or 26-30 bp in length. A DNA insert left and right border sequence are isolated from and/or native to the genome of a plant that is to be modified. A DNA insert border-like sequence is not identical in nucleotide sequence to any known Agrobacterium-derived T-DNA border sequence. Thus, a DNA insert border-like sequence may possess 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, or more nucleotides that are different from a T-DNA border sequence from an Agrobacterium species, such as Agrobacterium tumefaciens or Agrobacterium rhizogenes. That is, a DNA insert border, or a border-like sequence of the present invention has at least 95%, at least 90%, at least 80%, at least 75%, at least 70%, at least 60% or at least 50% sequence identity with a T-DNA border sequence from an Agrobacterium species, such as Agrobacterium tumefaciens or Agrobacterium rhizogenes, but not 100% sequence identity. As used herein, the descriptive terms “DNA insert border” and “DNA insert border-like” are exchangeable. A border-like sequence can be isolated from a plant genome and be modified or mutated to change the efficiency by which it is capable of integrating a nucleotide sequence into another nucleotide sequence. Other polynucleotide sequences may be added to or incorporated within a border-like sequence of the present invention. Thus, a DNA insert left border or a DNA insert right border may be modified so as to possess 5′- and 3′-multiple cloning sites, or additional restriction sites. A DNA insert border sequence may be modified to increase the likelihood that backbone DNA from the accompanying vector is not integrated into the plant genome.

Consisting essentially of. A composition “consisting essentially of” certain elements is limited to the inclusion of those elements, as well as to those elements that do not materially affect the basic and novel characteristics of the inventive composition. Thus, so long as the composition does not affect the basic and novel characteristics of the instant invention, that is, does not contain foreign DNA that is not from the selected plant species or a plant that is sexually compatible with the selected plant species, then that composition may be considered a component of an inventive composition that is characterized by “consisting essentially of” language.

Cotyledon. A cotyledon is a type of seed leaf. The cotyledon contains the food storage tissues of the seed.

Degenerate primer. A “degenerate primer” is an oligonucleotide that contains sufficient nucleotide variations that it can accommodate base mismatches when hybridized to sequences of similar, but not exact, homology.

Dicotyledon (dicot). A flowering plant whose embryos have two seed leaves or cotyledons. Examples of dicots include, but are not limited to, tobacco, tomato, potato, sweet potato, cassava, legumes including alfalfa and soybean, carrot, strawberry, lettuce, oak, maple, walnut, rose, mint, squash, daisy, and cactus.

DNA insert. According to the present invention, the DNA insert to be inserted into the genome of a plant comprises polynucleotide sequences native to that plant or has native genetic elements to that plant. In one example, for instance, the DNA insert from pSIM1278 of the potato variety Y9 of the present invention is a non-coding polynucleotide that is native to potato or wild potato, a potato sexually-compatible plant, that is stably integrated into the genome of the plant cells upon transformation and silences genes involved in the expression of black spot bruises, asparagine accumulation and senescence sweetening. The DNA insert preferably comprises two expression cassettes and is inserted into a transformation vector referred to as the pSIM1278 transformation vector. The first cassette comprises fragments of both the asparagine synthetase-1 gene (Asn1) and the polyphenol oxidase-5 gene (Ppo5), arranged as inverted repeats between the Agp promoter of the ADP glucose pyrophosphorylase gene (Agp) and the Gbss promoter of the granule-bound synthase gene (Gbss). These promoters are predominantly active in tubers. The function of the second cassette is to silence the promoters of the starch associated gene dikinase-R1 (R1) and the phosphorylase-L gene (PhL). This cassette is comprised of fragments of the promoters of the starch associated gene dikinase-R1 (R1) and the phosphorylase-L gene (PhL), operably linked to the same Agp and Gbss promoters as the first cassette. A second DNA insert comes from the transformation vector referred to as pSIM1678 that comprises the Rpi-vnt1 expression cassette and a silencing cassette for the plant vacuolar invertase gene, VInv. The Rpi-vnt1 gene cassette consists of the VNT1 protein coding region regulated by its native promoter and terminator sequences to confer broad resistance to late blight, whereas the silencing cassette consists of an inverted repeat of sequence from the potato VInv gene flanked by opposing plant promoters, pGbss and pAgp. These expression cassettes contain no foreign DNA, and consist of DNA only from either the selected plant species or from a plant that is sexually compatible with the selected plant species.

Embryo. The embryo is the immature plant contained within a mature seed.

Foreign. “Foreign,” with respect to a nucleic acid, means that that nucleic acid is derived from non-plant organisms, or derived from a plant that is not the same species as the plant to be transformed or is not derived from a plant that is not interfertile with the plant to be transformed, does not belong to the species of the target plant. According to the present invention, foreign DNA or RNA represents nucleic acids that are naturally occurring in the genetic makeup of fungi, bacteria, viruses, mammals, fish or birds, but are not naturally occurring in the plant that is to be transformed. Thus, a foreign nucleic acid is one that encodes, for instance, a polypeptide that is not naturally produced by the transformed plant. A foreign nucleic acid does not have to encode a protein product. According to the present invention, a desired intragenic plant is one that does not contain any foreign nucleic acids integrated into its genome.

Gene. As used herein, “gene” refers to the coding region and does not include nucleotide sequences that are 5′- or 3′- to that region. A functional gene is the coding region operably linked to a promoter or terminator. A gene can be introduced into a genome of a species, whether from a different species or from the same species, using transformation or various breeding methods.

Gene Converted (Conversion). Gene converted (conversion) plant refers to plants which are developed by a plant breeding technique called backcrossing wherein essentially all of the desired morphological and physiological characteristics of a variety are recovered in addition to the one or more genes transferred into the variety via the backcrossing technique, via genetic engineering or via mutation. One or more loci may also be transferred.

Genetic rearrangement. Refers to the re-association of genetic elements that can occur spontaneously in vivo as well as in vitro which introduce a new organization of genetic material. For instance, the splicing together of polynucleotides at different chromosomal loci, can occur spontaneously in vivo during both plant development and sexual recombination. Accordingly, recombination of genetic elements by non-natural genetic modification techniques in vitro is akin to recombination events that also can occur through sexual recombination in vivo.

Golden nematode. Globodera rostochiensis, commonly known as golden nematode, is a plant parasitic nematode affecting the roots and tubers of potato plants. Symptoms include poor plant growth, wilting, water stress and nutrient deficiencies.

Hypocotyl. A hypocotyl is the portion of an embryo or seedling between the cotyledons and the root. Therefore, it can be considered a transition zone between shoot and root.

In frame. Nucleotide triplets (codons) are translated into a nascent amino acid sequence of the desired recombinant protein in a plant cell. Specifically, the present invention contemplates a first nucleic acid linked in reading frame to a second nucleic acid, wherein the first nucleotide sequence is a gene and the second nucleotide is a promoter or similar regulatory element.

Integrate. Refers to the insertion of a nucleic acid sequence from a selected plant species, or from a plant that is from the same species as the selected plant, or from a plant that is sexually compatible with the selected plant species, into the genome of a cell of a selected plant species. “Integration” refers to the incorporation of only native genetic elements into a plant cell genome. In order to integrate a native genetic element, such as by homologous recombination, the present invention may “use” non-native DNA as a step in such a process. Thus, the present invention distinguishes between the “use of” a particular DNA molecule and the “integration” of a particular DNA molecule into a plant cell genome.

Introduction. As used herein, refers to the insertion of a nucleic acid sequence into a cell, by methods including infection, transfection, transformation or transduction.

Isolated. “Isolated” refers to any nucleic acid or compound that is physically separated from its normal, native environment. The isolated material may be maintained in a suitable solution containing, for instance, a solvent, a buffer, an ion, or other component, and may be in purified, or unpurified, form.

Late blight. A potato disease caused by the oomycete Phytophthora infestans and also known as ‘potato blight’ that can infect and destroy the leaves, stems, fruits, and tubers of potato plants.

Leader. Transcribed but not translated sequence preceding (or 5′ to) a gene.

Locus. A locus confers one or more traits such as, for example, male sterility, herbicide tolerance, insect resistance, disease resistance, waxy starch, modified fatty acid metabolism, modified phytic acid metabolism, modified carbohydrate metabolism, and modified protein metabolism. The trait may be, for example, conferred by a naturally occurring gene introduced into the genome of the variety by backcrossing, a natural or induced mutation, or a transgene introduced through genetic transformation techniques. A locus may comprise one or more alleles integrated at a single chromosomal location.

Marketable Yield. Marketable yield is the weight of all tubers harvested that are between 2 and 4 inches in diameter. Marketable yield is measured in cwt (hundred weight) where cwt=100 pounds.

Monocotyledon (monocot). A flowering plant whose embryos have one cotyledon or seed leaf. Examples of monocots include, but are not limited to turf grass, maize, rice, oat, wheat, barley, sorghum, orchid, iris, lily, onion, and palm.

Native. A “native” genetic element refers to a nucleic acid that naturally exists in, originates from, or belongs to the genome of a plant that is to be transformed. Thus, any nucleic acid, gene, polynucleotide, DNA, RNA, mRNA, or cDNA molecule that is isolated either from the genome of a plant or plant species that is to be transformed or is isolated from a plant or species that is sexually compatible or interfertile with the plant species that is to be transformed, is “native” to, i.e., indigenous to, the plant species. In other words, a native genetic element represents all genetic material that is accessible to plant breeders for the improvement of plants through classical plant breeding. Any variants of a native nucleic acid also are considered “native” in accordance with the present invention. In this respect, a “native” nucleic acid may also be isolated from a plant or sexually compatible species thereof and modified or mutated so that the resultant variant is greater than or equal to 99%, 98%, 97%, 96%, 95%, 94%, 93%, 92%, 91%, 90%, 89%, 88%, 87%, 86%, 85%, 84%, 83%, 82%, 81%, 80%, 79%, 78%, 77%, 76%, 75%, 74%, 73%, 72%, 71%, 70%, 69%, 68%, 67%, 66%, 65%, 64%, 63%, 62%, 61%, or 60% similar in nucleotide sequence to the unmodified, native nucleic acid isolated from a plant. A native nucleic acid variant may also be less than about 60%, less than about 55%, or less than about 50% similar in nucleotide sequence. A “native” nucleic acid isolated from a plant may also encode a variant of the naturally occurring protein product transcribed and translated from that nucleic acid. Thus, a native nucleic acid may encode a protein that is greater than or equal to 99%, 98%, 97%, 96%, 95%, 94%, 93%, 92%, 91%, 90%, 89%, 88%, 87%, 86%, 85%, 84%, 83%, 82%, 81%, 80%, 79%, 78%, 77%, 76%, 75%, 74%, 73%, 72%, 71%, 70%, 69%, 68%, 67%, 66%, 65%, 64%, 63%, 62%, 61%, or 60% similar in amino acid sequence to the unmodified, native protein expressed in the plant from which the nucleic acid was isolated.

Native genetic elements. “Native genetic elements” can be incorporated and integrated into a selected plant species genome according to the present invention. Native genetic elements are isolated from plants that belong to the selected plant species or from plants that are sexually compatible with the selected plant species. For instance, native DNA incorporated into cultivated potato (Solanum tuberosum) can be derived from any genotype of S. tuberosum or any genotype of a wild potato species that is sexually compatible with S. tuberosum (e.g., S. demissum).

Naturally occurring nucleic acid. Naturally occurring nucleic acid are found within the genome of a selected plant species and may be a DNA molecule or an RNA molecule. The sequence of a restriction site that is normally present in the genome of a plant species can be engineered into an exogenous DNA molecule, such as a vector or oligonucleotide, even though that restriction site was not physically isolated from that genome. Thus, the present invention permits the synthetic creation of a nucleotide sequence, such as a restriction enzyme recognition sequence, so long as that sequence is naturally occurring in the genome of the selected plant species or in a plant that is sexually compatible with the selected plant species that is to be transformed.

Operably linked. Combining two or more molecules in such a fashion that in combination they function properly in a plant cell. For instance, a promoter is operably linked to a structural gene when the promoter controls transcription of the structural gene.

Plant. As used herein, the term “plant” includes but is not limited to angiosperms and gymnosperms such as potato, tomato, tobacco, alfalfa, lettuce, carrot, strawberry, sugarbeet, cassava, sweet potato, soybean, maize, turf grass, wheat, rice, barley, sorghum, oat, oak, eucalyptus, walnut, and palm. Thus, a plant may be a monocot or a dicot. The word “plant,” as used herein, also encompasses plant cells, seed, plant progeny, propagule whether generated sexually or asexually, and descendents of any of these, such as cuttings or seed. Plant cells include suspension cultures, callus, embryos, meristematic regions, callus tissue, leaves, roots, shoots, gametophytes, sporophytes, pollen, seeds and microspores. Plants may be at various stages of maturity and may be grown in liquid or solid culture, or in soil or suitable media in pots, greenhouses or fields. Expression of an introduced leader, trailer or gene sequences in plants may be transient or permanent. A “selected plant species” may be, but is not limited to, a species of any one of these “plants.”

Plant Parts. As used herein, the term “plant parts” (or a potato plant, or a part thereof) includes but is not limited to protoplast, leaf, stem, root, root tip, anther, pistil, seed, embryo, pollen, ovule, cotyledon, hypocotyl, flower, tuber, eye, tissue, petiole, cell, meristematic cell, and the like.

Plant species. The group of plants belonging to various officially named plant species that display at least some sexual compatibility.

Plant transformation and cell culture. Broadly refers to the process by which plant cells are genetically modified and transferred to an appropriate plant culture medium for maintenance, further growth, and/or further development.

Precise breeding. Refers to the improvement of plants by stable introduction of nucleic acids, such as native genes and regulatory elements isolated from the selected plant species, or from another plant in the same species as the selected plant, or from species that are sexually compatible with the selected plant species, into individual plant cells, and subsequent regeneration of these genetically modified plant cells into whole plants. Since no unknown or foreign nucleic acid is permanently incorporated into the plant genome, the inventive technology makes use of the same genetic material that is also accessible through conventional plant breeding.

Progeny. As used herein, includes an F₁ potato plant produced from the cross of two potato plants where at least one plant includes potato cultivar Y9 and progeny further includes, but is not limited to, subsequent F₂, F₃, F₄, F₅, F₆, F₇, F₈, F₉, and Y9 generational crosses with the recurrent parental line.

Quantitative Trait Loci (QTL). Quantitative trait loci (QTL) refer to genetic loci that control to some degree numerically representable traits that are usually continuously distributed.

Recombinant. As used herein, broadly describes various technologies whereby genes can be cloned, DNA can be sequenced, and protein products can be produced. As used herein, the term also describes proteins that have been produced following the transfer of genes into the cells of plant host systems.

Regeneration. Regeneration refers to the development of a plant from tissue culture.

Regulatory sequences. Refers to those sequences which are standard and known to those in the art that may be included in the expression vectors to increase and/or maximize transcription of a gene of interest or translation of the resulting RNA in a plant system. These include, but are not limited to, promoters, peptide export signal sequences, introns, polyadenylation, and transcription termination sites. Methods of modifying nucleic acid constructs to increase expression levels in plants are also generally known in the art (see, e.g. Rogers et al., 260 J. Biol. Chem. 3731-38, 1985; Cornejo et al., 23 Plant Mol. Biol. 567: 81, 1993). In engineering a plant system to affect the rate of transcription of a protein, various factors known in the art, including regulatory sequences such as positively or negatively acting sequences, enhancers and silencers, as well as chromatin structure may have an impact. The present invention provides that at least one of these factors may be utilized in engineering plants to express a protein of interest. The regulatory sequences of the present invention are native genetic elements, i.e., are isolated from the selected plant species to be modified.

Selectable marker. A “selectable marker” is typically a gene that codes for a protein that confers some kind of resistance to an antibiotic, herbicide or toxic compound, and is used to identify transformation events. Examples of selectable markers include the streptomycin phosphotransferase (spt) gene encoding streptomycin resistance, the phosphomannose isomerase (pmi) gene that converts mannose-6-phosphate into fructose-6 phosphate; the neomycin phosphotransferase (nptII) gene encoding kanamycin and geneticin resistance, the hygromycin phosphotransferase (hpt or aphiv) gene encoding resistance to hygromycin, acetolactate synthase (als) genes encoding resistance to sulfonylurea-type herbicides, genes coding for resistance to herbicides which act to inhibit the action of glutamine synthase such as phosphinothricin or basta (e.g., the bar gene), or other similar genes known in the art.

Sense suppression. Reduction in expression of an endogenous gene by expression of one or more an additional copies of all or part of that gene in transgenic plants.

Specific gravity. As used herein, “specific gravity” is an expression of density and is a measurement of potato quality. There is a high correlation between the specific gravity of the tuber and the starch content and percentage of dry matter or total solids. A higher specific gravity contributes to higher recovery rate and better quality of the processed product.

T-DNA-Like. A “T-DNA-like” sequence is a nucleic acid that is isolated from a selected plant species, or from a plant that is sexually compatible with the selected plant species, and which shares at least 75%, 80%, 85%, 90%, or 95%, but not 100%, sequence identity with Agrobacterium species T-DNA. The T-DNA-like sequence may contain one or more border or border-like sequences that are each capable of integrating a nucleotide sequence into another polynucleotide.

Total Yield. Total yield refers to the total weight of all harvested tubers.

Trailer. Transcribed but not translated sequence following (or 3′ to) a gene.

Transcribed DNA. DNA comprising both a gene and the untranslated leader and trailer sequence that are associated with that gene, which is transcribed as a single mRNA by the action of the preceding promoter.

Transformation of plant cells. A process by which DNA is stably integrated into the genome of a plant cell. “Stably” refers to the permanent, or non-transient retention and/or expression of a polynucleotide in and by a cell genome. Thus, a stably integrated polynucleotide is one that is a fixture within a transformed cell genome and can be replicated and propagated through successive progeny of the cell or resultant transformed plant. Transformation may occur under natural or artificial conditions using various methods well known in the art. Transformation may rely on any known method for the insertion of nucleic acid sequences into a prokaryotic or eukaryotic host cell, including Agrobacterium-mediated transformation protocols, viral infection, whiskers, electroporation, heat shock, lipofection, polyethylene glycol treatment, micro-injection, and particle bombardment.

Transgene. A gene that will be inserted into a host genome, comprising a protein coding region. In the context of the instant invention, the elements comprising the transgene are isolated from the host genome.

Transgenic plant. A genetically modified plant which contains at least one transgene.

Variant. A “variant,” as used herein, is understood to mean a nucleotide or amino acid sequence that deviates from the standard, or given, nucleotide or amino acid sequence of a particular gene or protein. The terms, “isoform,” “isotype,” and “analog” also refer to “variant” forms of a nucleotide or an amino acid sequence. An amino acid sequence that is altered by the addition, removal or substitution of one or more amino acids, or a change in nucleotide sequence, may be considered a “variant” sequence. The variant may have “conservative” changes, wherein a substituted amino acid has similar structural or chemical properties, e.g., replacement of leucine with isoleucine. A variant may have “nonconservative” changes, e.g., replacement of a glycine with a tryptophan. Analogous minor variations may also include amino acid deletions or insertions, or both. Guidance in determining which amino acid residues may be substituted, inserted, or deleted may be found using computer programs well known in the art such as Vector NTI Suite (InforMax, MD) software.

Vine Maturity. Vine maturity refers to a plant's ability to continue to utilize carbohydrates and photosynthesize. Vine maturity is scored on a scale of 1 to 5 where 1=dead vines and 5=vines green, still flowering.

The insertion of desirable traits into the genome of potato plants presents particular difficulties because potato is tetraploid, highly heterozygous and sensitive to in-breeding depression. It is therefore very difficult to efficiently develop transgenic potato plants that produce less acrylamide and less harmful Maillard-reaction products, including N-Nitroso-N-(3-keto-1,2-butanediol)-3′-nitrotyramine (Wang et al., Arch Toxicol 70: 10-5, 1995), 5-hydroxymethyl-2-furfural (Janzowski et al., Food Chem Toxicol 38: 801-9, 2000), and other Maillard reaction products with mutagenic properties (Shibamoto, Prog Clin Biol Res 304: 359-76, 1989), during processing using conventional breeding.

Several methods have been tested and research is ongoing to reduce acrylamide through process changes, reduction in dextrose, and additives such as asparaginase, citrate, and competing amino acids. The required capital expense to implement process changes throughout the potato industry would cost millions of dollars. In addition to the expense, these process changes have significant drawbacks including potentially negative flavors associated with additives such as asparaginase or citrate. Typically, fry manufacturers add dextrose during processing of french fries to develop the desired golden brown color, but dextrose also increases the formation of acrylamide through the Maillard reaction. Significant reductions in acrylamide occur by merely omitting dextrose from the process; however, the signature golden brown colors must then be developed some other way (such as though the addition of colors like annatto) The use of alternate colors, results in an absence of the typical flavors that develop through those browning reactions. Another challenge with the use of additives to reduce reactants like asparagine is moisture migration that occurs during frozen storage with the resulting return of asparagine to the surface and increased acrylamide. Finally, the blackening that occurs after potatoes are bruised affects quality and recovery in processing French fries and chips. Damaged and bruised potatoes must be trimmed or are rejected before processing, resulting in quality challenges or economic loss.

The “native technology” strategy of the present invention addresses the need of the potato industry to improve the agronomic characteristics and nutritional value of potatoes by reducing the expression of polyphenol oxidase-5 (PPO-5), which is responsible for black spot bruise, the expression of asparagine synthetase-1 (Asn-1), which is responsible for the accumulation of asparagine, a precursor in acrylamide formation, reducing the expression of the enzyme vacuolar invertase, which converts sucrose into glucose and fructose, and/or the expression of phosphorylase-L and kinase-R1, which are enzymes associated with the accumulation of reducing sugars that normally react with amino acids, such as asparagine, and form toxic Maillard products, including acrylamide. The partial or complete silencing of these genes in tubers decreases the potential to produce acrylamide. Use of the native technology of the invention allows for the incorporation of desirable traits into the genome of commercially valuable potato plant varieties by transforming the potatoes only with “native” genetic material, that is genetic material obtained from potato plants or plants that are sexually-compatible with potato plants, that contains only non-coding regulatory regions, without the integration of any foreign genetic material into the plant's genome. Desirable traits include high tolerance to impact-induced black spot bruise, increased resistance to late blight infection, reduced formation of the acrylamide precursor asparagine and reduced accumulation of reducing sugars, with consequent decrease in accumulation of toxic Maillard products, including acrylamide, improved quality and food color control. The incorporation of these desirable traits into existing potato varieties is impossible to achieve through traditional breeding because potato is tetraploid, highly heterozygous and sensitive to inbreeding depression.

The non-coding potato plant DNA insert sequences used in the present invention are native to the potato plant genome and do not contain any Agrobacterium DNA. One of the DNA inserts preferably comprises two expression cassettes and is inserted into a transformation vector referred to as the pSIM1278 transformation vector. The first cassette comprises fragments of both the asparagine synthetase-1 gene (Asn1) and the polyphenol oxidase-5 gene (Ppo5), arranged as inverted repeats between the Agp promoter of the ADP glucose pyrophosphorylase gene (Agp) and the Gbss promoter of the granule-bound synthase gene (Gbss). These promoters are predominantly active in tubers. The function of the second cassette is to silence the promoters of the starch associated gene dikinase-R1 (R1) and the phosphorylase-L gene (PhL). This cassette is comprised of fragments of the promoters of the starch associated gene dikinase-R1 (R1) and the phosphorylase-L gene (PhL), operably linked to the same Agp and Gbss promoters as the first cassette. These expression cassettes contain no foreign DNA, and consist of DNA only from either the selected plant species or from a plant that is sexually compatible with the selected plant species. A second DNA insert comes from the transformation vector referred to as pSIM1678 that comprises the Rpi-vnt1 expression cassette and a silencing cassette for the plant vacuolar invertase gene, VInv. The Rpi-vnt1 gene cassette consists of the VNT1 protein coding region regulated by its native promoter and terminator sequences to confer broad resistance to late blight, whereas the silencing cassette consists of an inverted repeat of sequence from the potato VInv gene flanked by opposing plant promoters, pGbss and pAgp. The function of the first cassette is to confer resistance to late blight, while the function of the second cassette is to silence the vacuolar invertase gene, reducing glucose and fructose.

The commercially valuable potato plant variety used in the present invention is Atlantic. Atlantic is the parent variety for Y9. Plants are moderately large, with thick, upright stems, and slightly swollen, sparsely pubescent nodes. Leaves are bright, medium green, smooth, and moderately pubescent with prominent wings, large asymmetrical primary leaflets and numerous secondary and tertiary leaflets. Flowers are profuse with green, awl-shaped, pubescent calyx lobes, pale lavender corolla, orange anthers and abundant, viable pollen. The cultivar is tolerant to scab and Verticillium wilt, resistant to pinkeye, highly resistant to Race A of golden nematode, virus X, tuber net necrosis, and shows some resistance to black spot bruise. Tubers are susceptible to internal heat necrosis, particularly in sandy soils in warm, dry seasons. Hollow heart in the larger diameter tubers (diameter >4 inches) can be serious in some growing areas. Tubers are oval to round with light to heavy scaly netted skin, moderately shallow eyes, and white flesh. Tuber dormancy is medium-long. With high yield potential, high specific gravity and uniform tuber size and shape, Atlantic is the standard variety for chipping from the field or from very short-term storage (Webb et al. 1978). The variety is fertile and mainly grown in the Northeast and Southeast, especially for the production of chips.

The present invention provides a potato variety of significant market value—namely Atlantic—transformed with the transformation vector pSIM1278 followed by transformation with a second transformation vector pSIM1678, identified using the polymerase chain reaction rather than markers, and successfully propagated. Also provided are food products made from the tubers of the potato plant variety Y9 of the present invention. Potato cultivar Y9 has the following unique plant variety identifier with the Organization for Economic Cooperation and Development (OECD):

Targeted gene silencing with native DNA reduces the level of the RNA transcripts of the targeted genes in the tubers of the potato plant variety Y9. Potato cultivar Y9 contains expression cassettes that lower levels of reducing sugars in tubers by multiple mechanisms. Through the transformation with pSIM1278, silencing cassettes were introduced for the promoters of the starch associated gene (R1) and the phosphorylase-L gene (PhL), while transformation with pSIM1678 introduced a silencing cassette for the invertase gene (VInv; Ye et al., 2010). Together, these traits function by slowing the conversion of starch and sucrose to reducing sugars (glucose and fructose).

Thus, the tubers of the potato plant variety Y9 of the invention incorporate highly desirable traits, including a reduced ratio in free amide amino acids asparagine and glutamine, which is associated with reduced acrylamide formation upon frying or baking. Specifically, the potato variety Y9 of the present invention is characterized by two- to more than four-fold reduction in free-asparagine content, reduced discoloration associated with black spot bruise and increased resistance to late blight. Furthermore, the potato variety Y9 of the invention displays a delay in the degradation of starch into the reducing sugars glucose and fructose during storage. Impairment of starch-to-sugar conversion further reduces senescence sweetening and acrylamide formation and limits heat-induced browning.

Potato variety Y9 of the present invention is therefore extremely valuable in the potato industry and food market, as its tubers produce significantly less acrylamide upon heat processing and do not carry any potentially harmful foreign genes.

EXAMPLES

The present invention uses native technology to integrate native non-coding DNA into the genome of selected potato plant varieties to develop new intragenic potato plant varieties. The method includes trait identification, design of vectors, incorporation of vectors into Agrobacterium, selection of the recipient potato variety, plant transformation, evidence of absence of open reading frames, and confirmation that the new potato plant varieties contain only the native DNA. The potato cultivar Y9 of the present invention has a lowered potential to form acrylamide, lower amounts of sucrose and is more resistant to black spot bruise than its untransformed counterpart. Additionally, potato cultivar Y9 of the present invention has increased resistance to late blight.

Example 1: The pSIM1278 Transformation Vector Backbone

Plasmid pSIM1278 is a 19.7 kb binary transformation vector used to transform potatoes. This example shows the source of the genetic elements, the cloning steps for the backbone, and T-DNA sequences, and the order of the elements in the plasmid.

The plasmid backbone (FIG. 1 and Table 1) contains two well-characterized bacterial origins of replication. pVS1 (pVS1 Sta and Rep) enables maintenance of the plasmid in Agrobacterium, and pBR322 (pBR322 bom and ori) enables maintenance of the plasmid in Escherichia coli. The Agrobacterium DNA overdrive sequence enhances cleavage at the RB, and the E. coli. nptII gene is a bacterial kanamycin selectable marker. The backbone contains an expression cassette comprising the Agrobacterium isopentenyl transferase (ipt) gene flanked by the Ranger Russet potato polyubiquitin (Ubi7) promoter and the Ranger Russet potato polyubiquitin (Ubi3) terminator. The ipt cassette is a screenable phenotype used to select against plasmid backbone DNA integration in the host plant. When present in transformed plant tissue, overexpression of ipt results in the overproduction of the plant hormone cytokinin resulting in plants with stunted phenotypes, abnormal leaves and the inability to root.

The backbone portion is not transferred into the plant cells. The various elements of the backbone are described in Table 1.

TABLE 1 Genetic Elements of the pSIM1278 Backbone Accession Size Genetic Element Origin Number¹ Position (bp) Function 1. Intervening sequence Synthetic DNA 10,149-10,154 6 Sequence used for cloning 2. Overdrive Agrobacterium NC_002377 10,155-10,187 33 Enhances cleavage of tumefaciens A. tumefaciens Right Border site¹ Ti-plasmid 3. Intervening sequence Pseudomonas AJ537514 10,188-11,266 1,079 pVS1 backbone¹ fluorescens pVS1 4. pVS1 partitioning P. fluorescens AJ537514 11,267-12,267 1,001 pVS1 stability¹ protein StaA (PVS1 Sta) pVS1 5. Intervening sequence P. fluorescens AJ537514 12,268-12,860 593 pVS1 backbone¹ pVS1 6. pVS1 replicon P. fluorescens AJ537514 12,861-13,861 1,001 pVS1 replication region in (pVS1Rep) pVS1 Agrobacterium ¹ 7. Intervening sequence P. fluorescens AJ537514 13,862-14,099 238 pVS1 backbone¹ pVS1 8. Intervening sequence pBR322 J01749 14,100-14,180 81 pBR322 backbone¹ 9. pBR322 bom pBR322 J01749 14,181-14,531 351 pBR322 region for replication in E. coli ¹ 10. Intervening sequence pBR322 J01749 14,532-14,670 139 pBR322 backbone¹ 11. Origin of replication pBR322 J01749 14,671-14,951 281 Bacterial origin of replication¹ for pBR322 (pBR322 ori) 12. Intervening sequence pBR322 J01749 14,952-15,241 290 pBR322 backbone¹ 13. Neomycin Tn5 transposon FJ362602 15,242-16,036 795 Aminoglycoside phosphotransferase II phosphotransferase¹ (Simpson et al. (nptII) gene 1985) 14. Intervening sequence Vector DNA FJ362602 16,037-16,231 195 pCAMBIA vector backbone¹ 15. Terminator of the S. tuberosum GP755544 16,232-16,586 355 Terminator for ipt gene transcription ubiquitin-3 gene (tUbi3) (Garbarino and Belknap, 1994) 16. Intervening sequence A. tumefaciens NC_002377 16,587-16,937 351 Sequence used for DNA cloning Ti-plasmid 17. Isopentenyl A. tumefaciens NC_002377 16,938-17,660 723 Condensation of AMP and transferase (ipt) gene Ti-plasmid isopentenyl-pyrophosphate to form isopentenyl-AMP, a cytokinin in the plant. Results in abnormal growth phenotypes in plant (Smigocki and Owens, 1988) 18. Intervening sequence Synthetic DNA 17,661-17,672 12 Sequence used for DNA cloning 19. Polyubiquitin S. tuberosum U26831 17,673-19,410 1,738 Promoter to drive expression of the promoter (Ubi7) var. Ranger ipt backbone marker gene Russet (Garbarino et al., 1995) 20. Intervening sequence Vector DNA U10460 19,411-19,660 250 pZP200 vector backbone¹ ¹http://www.cambia.org/daisy/cambia/585.html - (General structure map of pCAMBIA vectors)

Example 2: The pSIM1278 Transformation Vector T-DNA

The pSIM1278 DNA insert region, including the flanking border sequences, used in the pSIM1278 is 10,148 bp long, from 1 bp to 10,148 bp. The pSIM1278 DNA insert consists of native DNA only and is stably integrated into the potato genome. The pSIM1278 DNA insert or a functional part thereof, is the only genetic material of vector pSIM1278 that is integrated in the potato plant varieties of the invention.

The pSIM1278 DNA insert is described in: FIG. 1 (along with vector backbone region), FIG. 2, and Table 2 below. The LB and RB sequences (25 bp each) were synthetically designed to be similar to and function like T-DNA borders from Agrobacterium tumefaciens. The GenBank Accession AY566555 was revised to clarify the sources of DNA for the Border regions. ASN1 described as genetic elements 5 and 10 is referred to as StAst1 in Chawla et al., 2012.

Plasmid pSIM1278 T-DNA Contains Two Expression Cassettes:

The first cassette (elements 4 to 12, Table 2) results in down-regulation of Asn1 and Ppo5 in the transformed potato variety. It is comprised of two identical 405 bp fragments of Asn1 and two identical 144 bp fragments of Ppo5. The fragments of Asn1 and Ppo5 are arranged as inverted repeats separated by a non-coding 157 bp Ranger Russet potato nucleotide spacer element. The Asn1 and Ppo5 fragments are arranged between the two convergent potato promoters; the Agp promoter of the ADP glucose pyrophosphorylase gene (Agp) and the Gbss promoter of the granule-bound starch synthase gene (Gbss) that are primarily active in tubers. These promoters drive expression of the inverted repeats to generate double-stranded RNA and down-regulate Asn1 and Ppo5.

The second cassette (elements 14 to 21, Table 2) results in down-regulation of PhL and R1 in the transformed potato variety. It is comprised of two identical 509 bp fragments of the PhL promoter region (pPhL) and two identical 532 bp fragments of R1 promoter region (pR1). The pPhL and pR1 fragments are arranged as inverted repeats separated by a non-coding 258 bp fragment of the Ranger Russet potato polyubiquitin gene. Like the first cassette, the pPhL and pR1 fragments are arranged between and transcribed by the potato Agp and Gbss promoters.

TABLE 2 Genetic Elements of pSIM1278 T-DNA, from Left Border Site to Right Border Accession Position Size Genetic Element Origin Number (pSIM1278) (bp) Intended Function 1. Left Border (LB) site¹ Synthetic AY566555⁵  1-25 25 Site for secondary cleavage to release (bases 1-25) single-stranded DNA insert from pSIM1278 (van Haaren et al. 1989) 2. Left Border region S. tuberosum AY566555⁵  26-187 162 Supports secondary cleavage at LB sequence including LB var. Ranger (bases 26-187) Russet. 3. Intervening Sequence S. tuberosum AF393847 188-193 6 Sequence used for DNA cloning 4. Promoter for the ADP S. tuberosum HM363752  194-2,453 2260 One of the two convergent promoters that glucose pyrophosphorylase var. Ranger drives expression of an inverted repeat gene (pAgp), 1st copy Russet containing fragments of Asn1 and Ppo5, especially in tubers 5. Fragment of the S. tuberosum HM363759 2,454-2,858 405 Generates with (10) double stranded RNA asparagine synthetase-1 var. Ranger that triggers the degradation of Asn1 (Asn1) gene (1st copy Russet transcripts to impair asparagine formation antisense orientation) (Chawla et al., 2012²) 6. 3′-untranslated sequence S. verrucosum HM363754 2,859-3,002 144 Generates with (9) double stranded RNA of the polyphenol oxidase- that triggers the degradation of Ppo5 5 gene (Ppo5) (1st copy, in transcripts to block black spot antisense orientation) development 7. Intervening Sequence S. tuberosum DQ478950 3,003-3,008 6 Sequence used for DNA cloning 8. Spacer-1 S. tuberosum HM363753 3,009-3,165 157 Sequence between the 1st inverted repeats var. Ranger Russet 9. 3′-untranslated sequence S. verrucosum HM363754 3,166-3,309 144 Generates with (6) double stranded RNA of the polyphenol oxidase- that triggers the degradation of Ppo5 5 gene (Ppo5) (2nd copy, transcripts to block black spot in sense orientation) development 10. Fragment of the S. tuberosum HM363759 3,310-3,715 406 Generates with (5) double stranded RNA asparagine synthetase-1 var. Ranger that triggers the degradation of Asn1 (Asn1) gene (2nd copy, in Russet transcripts to impair asparagine formation sense orientation) (Chawla et al., 2012²) 11. Intervening Sequence S. tuberosum X73477 3,716-3,721 6 Sequence used for DNA cloning 12. Promoter for the S. tuberosum HM363755 3,722-4,407 686 One of the two convergent promoters that granule-bound starch var. Ranger drives expression of an inverted repeat synthase (pGbss) gene (1st Russet containing fragments of Asn1 and Ppo5, copy, convergent especially in tubers orientation relative to the 1st copy of pAgp) 13. Intervening Sequence S. tuberosum X95996/ 4,408-4,423 16 Sequence used for DNA cloning AF393847 14. pAgp, 2nd copy S. tuberosum HM363752 4,424-6,683 2260 One of the two convergent promoters that var. Ranger drives expression of an inverted repeat Russet containing fragments of the promoters of PhL and R1, especially in tubers 15. Fragment of promoter S. tuberosum HM363758 6,684-7,192 509 Generates with (20) double stranded RNA for the potato var. Ranger that triggers the degradation of PhL phosphorylase-L (pPhL) Russet transcripts to limit the formation of gene (1st copy, in reducing sugars through starch antisense orientation) degradation 16. Fragment of promoter S. tuberosum HM363757 7,193-7,724 532 Generates with (19) double stranded RNA for the potato R1 gene var. Ranger that triggers the degradation of R1 (pR1) (1st copy, in Russet transcripts to limit the formation of antisense orientation) reducing sugars through starch degradation 17. Intervening Sequence S. tuberosum DQ478950 7,725-7,730 6 Sequence used for DNA cloning 18. Spacer-2 S. tuberosum U26831³ 7,731-7,988 258 Sequence between the 2nd inverted repeat var. Ranger Russet 19. Fragment of promoter S. tuberosum HM363757 7,989-8,520 532 Generates with (16) double stranded RNA for the potato R1 gene var. Ranger that triggers the degradation of R1 (pR1) (2nd copy, in sense Russet transcripts to limit the formation of orientation) reducing sugars through starch degradation 20. Fragment of promoter S. tuberosum HM363758 8,521-9,029 509 Generates with (15) double stranded RNA for the potato var. Ranger that triggers the degradation of PhL phosphorylase-L (pPhL) Russet transcript to limit the formation of gene (2nd copy, in sense reducing sugars through starch orientation) degradation 21. pGbss (2nd copy, S. tuberosum X83220⁴ 9,030-9,953 924 One of the two convergent promoters that convergent orientation var. Ranger drives expression of an inverted repeat relative to the 2nd copy of Russet containing fragments of the promoters of pAgp) PhL and R1, especially in tubers 22. Intervening Sequence S. tuberosum AF143202 9,954-9,962 9 Sequence used for DNA cloning 23. Right Border region S. tuberosum AY566555⁵  9,963-10,123 161 Supports primary cleavage at RB-Like site sequence including RB var. Ranger (bases 231- Russet 391) 24. Right Border (RB) Synthetic AY566555⁵ 10,124-10,148 25 Site for primary cleavage to release single sequence¹ (bases 392- stranded DNA insert from pSIM1278 (van 416) Haaren et al. 1989) ¹The LB and RB sequences (25-bp each) were synthetically designed to be similar to and function like T-DNA borders from Agrobacterium tumefaciens. ²ASN1 described as genetic elements 5 and 11 is referred to as StAst1 in Chawla et al. 2012. ³GenBank Accession HM363756 is replaced with a citation to GenBank Accession U26831 to properly include four 3′ end nucleotides present in the pGbss DNA element of the pSIM1278 construct. ⁴GenBank Accession HM363755 is replaced with a citation to GenBank Accession X83220 to properly include the full pGbss (2nd copy) DNA insert sequence present in the pSIM1278 construct. ⁵GenBank Accession AY566555 was revised to clarify the sources of DNA for the Border regions.

Thus, as can be seen from Table 1 and Table 2, the pSIM1278 plasmid is a binary vector designed for potato plant transformation. The vector backbone contains sequences for replication in both E. coli and Agrobacterium along with an ipt marker for screening to eliminate plants with vector backbone DNA. The T-DNA region consists of two expression cassettes flanked by LB and RB sequences. Upon inoculation of host plant tissue with Agrobacterium containing the pSIM1278 vector, the T-DNA region of pSIM1278 is transferred into the host genome.

The DNA insert described in Table 2 that was used to create potato cultivar Y9 of the present disclosure does not activate adjacent genes and does not adversely affect the phenotype of potato plant varieties.

Example 3: The pSIM1678 Transformation Vector Backbone

Plasmid pSIM1678 is a 18.6 kb binary transformation vector used to transform potatoes. This example shows the source of the genetic elements, the cloning steps for the backbone, and T-DNA sequences, and the order of the elements in the plasmid.

The plasmid backbone (FIG. 3; Table 3) contains two well-characterized bacterial origins of replication. pVS1 (pVS1 Sta and Rep) enables maintenance of the plasmid in Agrobacterium, and pBR322 (pBR322 bom and ori) enables maintenance of the plasmid in Escherichia coli. The Agrobacterium DNA overdrive sequence enhances cleavage at the RB, and the E. coli. nptII gene is a bacterial kanamycin selectable marker. The backbone contains an expression cassette comprising the Agrobacterium isopentenyl transferase (ipt) gene flanked by the Ranger Russet potato polyubiquitin (Ubi7) promoter and the Ranger Russet potato polyubiquitin (Ubi3) terminator (Garbarino and Belknap, 1994). The ipt cassette is a screenable phenotype used to select against plasmid backbone DNA integration in the host plant. When present in transformed plant tissue, overexpression of ipt results in the overproduction of the plant hormone cytokinin resulting in plants with stunted phenotypes, abnormal leaves and the inability to root.

The backbone portion is not transferred into the plant cells. The various elements of the backbone are described in Table 3.

TABLE 3 Genetic Elements of the pSIM1678 Backbone Accession Size Genetic Element Origin Number¹ Position (bp) Function 1. Intervening sequence Synthetic DNA 9,091-9,096 6 Sequence used for cloning 2. Overdrive Agrobacterium NC_002377 9,097-9,126 30 Enhances cleavage of A. tumefaciens tumefaciens Right Border site¹ Ti-plasmid 3. Intervening sequence Pseudomonas AJ537514  9,127-10,208 1,082 pVS1 backbone¹ fluorescens pVS1 4. pVS1 partitioning protein P. fluorescens AJ537514 10,209-11,209 1,001 pVS1 stability¹ StaA (PVS1 Sta) pVS1 5. Intervening sequence P. fluorescens AJ537514 11,210-11,802 593 pVS1 backbone¹ pVS1 6. pVS1 replicon P. fluorescens AJ537514 11,803-12,803 1,001 pVS1 replication region in (pVS1Rep) pVS1 Agrobacterium ¹ 7. Intervening sequence P. fluorescens AJ537514 12,804-13,040 237 pVS1 backbone¹ pVS1 8. Intervening sequence pBR322 J01749 13,041-13,212 172 pBR322 backbone¹ 9. pBR322 bom pBR322 J01749 13,213-13,473 261 pBR322 region for replication in E. coli ¹ 10. Intervening sequence pBR322 J01749 13,474-13,612 139 pBR322 backbone¹ 11. Origin of replication for pBR322 J01749 13,613-13,893 281 Bacterial origin of replication¹ pBR322 (pBR322 ori) 12. Intervening sequence pBR322 J01749 13,894-14,183 290 pBR322 backbone¹ 13. Neomycin Tn5 transposon FJ362602 14,184-14,978 795 Aminoglycoside phosphotransferase¹ phosphotransferase II (nptII) (Simpson et al. 1985) gene 14. Intervening sequence Vector DNA FJ362602 14,979-15,173 195 pCAMBIA vector backbone¹ 15. Terminator of the S. tuberosum GP755544 15,174-15,528 355 Terminator for ipt gene transcription ubiquitin-3 gene (tUbi3) (Garbarino and Belknap, 1994) 16. Intervening sequence A. tumefaciens NC_002377 15,529-15,879 351 Sequence used for DNA cloning Ti-plasmid 17. Isopentenyl transferase A. tumefaciens NC_002377 15,880-16,602 723 Condensation of AMP and isopentenyl- (ipt) gene Ti-plasmid pyrophosphate to form isopentenyl- AMP, a cytokinin in the plant. Results in abnormal growth phenotypes in plant (Smigocki and Owens, 1988) 18. Intervening sequence Synthetic DNA 16,603-16,614 12 Sequence used for DNA cloning 19. Polyubiquitin promoter S. tuberosum var. (A)U26831 16,615-18,352 1,738 Promoter to drive expression of the ipt (Ubi7) Ranger Russet backbone marker gene (Garbarino et al., 1995) 20. Intervening sequence Vector DNA (B)U10460 18,353-18,602 250 pZP200 vector backbone ¹http://www.cambia.org/daisy/cambia/585.html - (General structure map of pCAMBIA vectors)

Example 4: The pSIM1678 Transformation Vector T-DNA

The pSIM1678 DNA insert region, including the flanking border sequences, used in the pSIM1678 is 9,090 bp long (from 1 bp to 9,090 bp). The pSIM1678 DNA insert consists of native DNA only and is stably integrated into the potato genome. The pSIM1678 DNA insert or a functional part thereof, is the only genetic material of vector pSIM1678 that is integrated in the potato plant varieties of the invention.

The pSIM1678 DNA insert is described in FIG. 3 (along with vector backbone region) and Table 4 below. In Table 4, the LB and RB sequences (25-bp each) were synthetically designed to be similar to and function like T-DNA borders from Agrobacterium tumefaciens. GenBank Accession AY566555 was revised to clarify the sources of DNA for the Border regions.

Plasmid pSIM1678 T-DNA is from 1-bp to 9,090-bp and contains two expression cassettes (FIG. 3):

The first cassette (elements 4 to 6, Table 4) contains the 2,626 bp Rpi-vnt1 (Vnt1) gene originating from Solanum venturii. The gene product, VNT1, is an R-protein involved in the plant immune response that protects potato from late blight infection from Phytophthora infestans. The gene is expressed under the native Vnt1 promoter, pVnt1, and terminator, tVnt1.

The second cassette (elements 8 to 14, Table 4) results in down-regulation of vaculor Invertase (VInv) in the transformed potato variety. It is comprised of two fragments of VInv (elements 10 and 12, Table 4) arranged as inverted repeats separated. VInv fragments are arranged between the two convergent potato promoters; the Agp promoter of the ADP glucose pyrophosphorylase gene (Agp) and the Gbss promoter of the granule-bound starch synthase gene (Gbss) that are primarily active in tubers. These promoters drive expression of the inverted repeats to generate double-stranded RNA and down-regulate VInv.

TABLE 4 Genetic Elements of pSIM1678 T-DNA, from Left Border Site to Right Border Accession Position Size Genetic Element Origin Number (pSIM1678) (bp) Intended Function 1. Left Border (LB) Synthetic AY566555³  1-25 25 Site for secondary cleavage site¹ (bases 1-25) to release single-stranded DNA insert from pSIM1678 2. Left Border region S. tuberosum AY566555³  26-187 162 Supports secondary sequence including LB var. Ranger (bases 1-187) cleavage at LB Russet. 3. Intervening Sequence S. tuberosum AF393847 188-193 6 Sequence used for DNA cloning 4. Native promoter for S. venturii FJ423044 194-902 709 Drives expression of late the late blight resistance blight resistance gene vnt1 gene (Vnt1) 5. Late blight resistance S. venturii FJ423044  903-3,578 2676 Solarium venturii late blight gene VNt1 (Rpi-vnt1) resistance protein gene 6. Native terminator for S. venturii FJ423044 3,579-4,503 925 Ends transcription of late the Vnt1 gene blight resistance gene vnt1 7. Intervening Sequence S. tuberosumt HM363755 4,504-4,510 7 Sequence used for DNA cloning 8. Promoter for the S. tuberosum HM363752 4,511-6,770 2260 One of the two convergent ADP glucose var. Ranger promoters that drives pyrophosphorylase gene Russet expression of an inverted (pAgp) repeat containing fragments of acid invertase gene 9. Intervening Sequence S. tuberosum DQ206630 6,771-6,776 6 Sequence used for DNA var. Ranger cloning Russet 10. Fragment of the acid S. tuberosum DQ478950 6,777-7,455 679 Generates with (12) double invertase (Inv) (sense var. Ranger stranded RNA that triggers orientation) Russet the degradation of invertase transcripts 11. Intervening S. tuberosum X73477 7,456-7,461 6 Sequence used for DNA Sequence var. Ranger cloning Russet 12. Fragment of the acid S. tuberosum DQ478950 7,462-7,965 504 Generates with (10) double invertase (Inv) (anti- var. Ranger stranded RNA that triggers sense orientation) Russet the degradation of invertase transcripts 13. Intervening S. tuberosum X95996 7,966-7,971 6 Sequence used for DNA Sequence var. Ranger cloning Russet 14. Promoter for the S. tuberosum X83220² 7,972-8,895 924 One of the two convergent granule-bound starch var. Ranger promoters that drives synthase (pGbss) gene Russet expression of an inverted (convergent orientation repeat containing fragments relative to the pAgp) of invertase gene, especially in tubers 15. Intervening S. tuberosum AF143202 8,896-8904  9 Sequence used for DNA Sequence cloning 16. Right Border region S. tuberosum AY566555³  8905-9,065 161 Supports primary cleavage sequence including RB var. Ranger (bases 231- at RB-Like site Russet 416) 17. Right Border (RB) Synthetic AY566555³ 9,066-9,090 25 Site for primary cleavage to sequence¹ (bases 392- release single stranded DNA 416) insert from pSIM1678 (van Haaren et al., 1989) ¹The LB and RB sequences (25-bp each) were synthetically designed to be similar to and function like T-DNA borders from Agrobacterium tumefaciens. ²GenBank Accession HM363755 is replaced with a citation to GenBank Accession X83220 to properly include the full pGbss (2nd copy) DNA insert sequence present in the pSIM1278 construct. ³GenBank Accession AY566555 was revised to clarify the sources of DNA for the Border regions.

Thus, as can be seen from Table 3 and Table 4, the pSIM1678 plasmid is a binary vector designed for potato plant transformation. The vector backbone contains sequences for replication in both E. coli and Agrobacterium along with an ipt marker for screening to eliminate plants with vector backbone DNA. The T-DNA region consists of two expression cassettes flanked by LB and RB sequences. Upon inoculation of host plant tissue with Agrobacterium harboring the pSIM1678 vector, the T-DNA region of pSIM1678 is transferred into the host genome.

Example 5: The Agrobacterium Strain and Transfection

The C58-derived Agrobacterium strain AGL1 was developed by precisely deleting the transfer DNA of the hyper-virulent plasmid pTiBo542 (Lazo et al., 1991). A transposon insertion in the general recombination gene (recA) stabilizes recombinant plasmid vectors such as pSIM1278 (FIG. 1). AGL1 displays resistance against carbenicillin and rifampicin, and is eliminated from transformed potato tissue using timentin. Following selection, plants are both antibiotic and Agrobacterium free, with the potato-derived expression cassettes inserted into the plant's genome.

Stock plants were maintained in magenta boxes with 40 ml half-strength M516 (Phytotechnology) medium containing 3% sucrose and 2 g/l gelrite (propagation medium). Potato internode segments of four to six mm were cut from four-week old plants, infected with the Agrobacterium AGL1 strain carrying pSIM1278, and transferred to tissue culture media containing 3% sucrose and 6 g/l agar (co-cultivation medium). Infected explants were transferred, after two days, to M404 (Phytotechnology) medium containing 3% sucrose, 6 g/l agar and 150 mg/l timentin to eliminate Agrobacterium (hormone-free medium). Details of the methods are described in Richael et al. (2008).

After one month, the infected explants were transferred to fresh medium lacking any synthetic hormones and incubated in a Percival growth chamber under a 16 hr photoperiod at 24° C. where they started to form shoots. Many shoots expressed the ipt gene and displayed a cytokinin overproduction phenotype; these shoots were not considered for further analyses. PCR genotyping demonstrated that about 0.3 to 1.5% of the remaining shoots contained at least part of the P-DNA while lacking the ipt gene. Thus, no markers were used to select for the transformed plants. Details on ipt-based marker-free plant transformation were published by Richael et al. (2008).

The process of eliminating Agrobacterium started two days after explant infection. For this purpose, tissues were subjected to the antibiotic timentin (150 mg/L) until proven to be free of live Agrobacterium. Proof was obtained by incubating stem fragments of transformed events on nutrient broth-yeast extract (NBY medium) for 2 weeks at 28° C. (repeated twice). In accordance with 97 CFR Part 340, transformed plants were transported and planted in the field only when free of live Agrobacterium.

The Atlantic Y9 event contains inserts derived from two separate transformations with different plasmids. The first insert, plasmid pSIM1278, contains two cassettes consisting of inverted repeats designed to silence up to four potato genes, Asn1, Ppo5, R1, and PhL, in tubers. Similarly, the second plasmid, pSIM1678, contains a cassette consisting of an inverted repeat to silence the VInv gene in tubers, while also containing a copy of the Rpi-vnt1 gene under its native potato promoter.

Potato plant varieties were analyzed by DNA gel blot analyses to determine the structure and copy number of integrated DNA insert sequences and to confirm the absence of vector backbone sequences.

Example 6: Evidence for the Absence of the Vector Backbone DNA

Unlike many commercial transgenic crops, potato cultivars of the disclosure were confirmed to be free of Agrobacterium-derived DNA sequences that are used for transformation, such as vector backbone DNA, by two different methods: 1) First, the presence or absence of the negative selectable isopentenyl isomerase (ipt) marker gene in the vector backbone was determined, as inadvertent transfer of backbone DNA comprising the ipt gene expression cassette from Agrobacterium to plant cells would trigger ipt gene expression and, consequently, the formation of the cytokinin-type hormone isopentenyladenosine, if plants had phenotypes associated with the negative selectable isopentenyl isomerase (ipt) marker gene in the plasmid backbone, they were discarded; and 2) Southern blot hybridization was then used on the transformed potato plants that had passed the first screening method to confirm the absence of backbone DNA.

Thus, the above two analyses have shown that the Atlantic Y9 event does not contain backbone from either plasmid used in the transformations.

Example 7: Stability of the Inserted DNA

Bacterial T-DNAs are not always stable after insertion into a plant. The estimated instability rate (0.5-5.9×10⁻⁴) is associated with meiosis (Müllner et al. 1987; Conner et al. 1998), which is not relevant to potatoes as they reproduce vegetatively. Thus, DNA insertions are expected to be stable. Tubers rather than seeds were used to define subsequent generations since tubers are what are commercially planted.

Genetic stability was assessed using molecular and phenotypic assays. The structure of the insert was shown to be stable using Southern blot analysis of genomic DNA isolated over three generations of Y9 potatoes (G0-G3), whereas the phenotypic stability was assessed by measuring polyphenol oxidase activity, in the second generation of field-grown tubers. This method shows visual evidence of PPO silencing after applying catechol to the cut surface of potatoes. These studies were carried out to ensure that the desired genetic changes in Y9 remained stable over multiple clonal cycles while maintaining the traits.

The stability of the DNA inserts was evaluated by comparing three successive clonal generations (G1, G2, and G3) to the original transformant (G0) using Southern blots. Stable DNA inserts are expected to maintain the same structure and thus produce the same digestion patterns over multiple generations of the plant. To test stability of the inserts in the Y9 event, its digestion pattern was compared using two probes (GBS1 and AGP) that hybridize to regions of the inserts from both pSIM1278 and pSIM1678, and two probes (INV and VNT1) that are specific to the pSIM1678 insert. Since the DNA sequences these probes hybridize with are contained in the potato genome as well as within the DNA insert(s), both endogenous and insert-specific bands are expected in the Southern blots.

All genomic DNA samples were digested with the restriction enzyme, EcoRV, and hybridized with a probe specific to either AGP or GBS1. EcoRV was chosen for these studies as it digests within both inserts to provide a unique banding pattern with internal bands of predicted size in the pSIM1278 insert (e.g. 2.3 kb). The banding patterns between all samples of Y9 were identical to each other for both probes. The multiple bands present in the Atlantic control are also found in Y9, but Y9 also contains bands corresponding to the pSIM1278 and pSIM1678 inserts. These bands are similarly consistent between all generations of Y9 analyzed indicating genetic stability of both inserts.

A second analysis was performed using two probes specific to the pSIM1678 insert. For this analysis, genomic DNA samples were digested with the restriction enzyme, XbaI, and hybridized with VNT1 and INV probes. XbaI was chosen as the restriction enzyme for these studies as it digests the pSIM1678 internally and produces a band of known size (e.g. 4.6 kb for the INV probe). Again, both endogenous and insert-specific bands were detected with consistent banding patterns between the three generations analyzed. The genetic and phenotypic analyses indicated the insertions arising from transformation of both pSIM1278 and pSIM1678 are stable over three generations. Given the demonstrated stability over three generations, it is likely that stability will be maintained during subsequent cycles of vegetative propagation.

Example 8: Efficacy and Tissue-Specificity of Gene Silencing

Silencing was achieved by introducing inverted repeats containing sequences derived from the genes and promoters targeted for silencing. Although there are a number of parallel pathways involved in double-stranded RNA mediated silencing, transcription of these inverted repeats is thought to be processed by the cellular machinery involved in the viral defense (Fusaro et al. 2006). Y9 potatoes contain three unique cassettes, which contain sequence from a total of five different potato genes. The pSIM1278 construct consists of two gene silencing cassettes (see FIG. 4, upper construct). One cassette contains an inverted repeat of sequence from two genes, asparagine synthetase-1 (Asn1) and polyphenol oxidase-5 (Ppo5). The second cassette includes sequence from the promoters of the starch associated genes, R1 (531-bp) and phosphorylase-L (PhL) (508-bp). The final cassette was introduced through the pSIM1678 construct, which includes an inverted repeat containing sequence from the vacuolar invertase (VInv) gene (see FIG. 4, lower construct).

All three silencing cassettes are regulated by the same set of well-characterized and tissue-specific promoters from the Agp and Gbss genes of potato, which are highly active in tubers compared with photosynthetically-active tissues and roots (Nakata et al. 1994; Visser et al. 1991). Therefore, expression and gene silencing was expected to be most effective in and largely limited to tubers.

The expression of all five target genes was characterized by northern blot analysis to determine the effectiveness of gene silencing from each cassette. And, as shown by Table 5 below, all five genes were shown to be down-regulated in tubers.

TABLE 5 Summary of RNAi-Target Gene Expression in Y9 Tissues Gene Tuber Leaf Stem Root Flower Asn1  ✓¹ ✓ — — ✓ Ppo5 ✓ — — — — PhL ✓ — — — — R1 ✓ — — — — VInv ✓ — — — ✓ ¹✓ = down-regulated, — = not down-regulated, n/o = not observed.

Tuber-specific down-regulation of Asn1, Ppo5, PhL, R1, and VInv genes was observed in the Y9 event. Expression levels in other tissues were unaffected, except for partial down-regulation of Asn1 in leaves and Asn1 and VInv in flowers.

Example 9: Potato Cultivar Y9 Characterization Summary

Potato variety Y9 addresses the need of the potato industry to improve quality by increasing resistance to late blight, reducing expression of the enzyme responsible for black spot bruise and to reduce acrylamide through lowering the concentration of the reactants, namely asparagine and reducing sugars. Potato variety Y9 was transformed with nucleic acid sequences that are native to the potato plant genome and does not contain foreign DNA, Agrobacterium DNA, viral markers or vector backbone sequences In addition, agronomic studies were conducted to ensure that the events grew the same as conventional controls, with the exception of the characteristics associated with the trait

Field trials were conducted at seven U.S. sites during 2014. The purpose of this study was to evaluate the phenotypic performance, tubers, and ecological interactions of Y9 potatoes compared with an untransformed control, the parental variety, Atlantic.

The phenotypic, tuber, and ecological interactions studies did not indicate any meaningful differences between Y9 and the Atlantic control.

There were no statistical differences detected for any of the phenotypic characteristics, indicating that Y9 is comparable to Atlantic in terms of phenotype.

For the tuber assessment, specific gravity was higher for Y9 compared to the control, but within the range of values seen in conventional potatoes. This change would not alter the environmental impact of Y9 which is the same as conventional potatoes.

The lack of differences for insect, disease, and abiotic stressors, as well as arthropod abundance, supports a conclusion that the ecological interactions of Y9 are the same as conventional potatoes.

TABLE 6 Phenotypic, Yield, and Grading Characteristics CVR CVR Characteristic Variety N Mean P-Value SD Min Max Phenotypic Performance Early Emergence (%) Atlantic Ctrl 28 72.1 0.3276 22.7 0 100 Y9 28 67.2 20.5 Final Emergence (%) Atlantic Ctrl 28 96.0 0.4245 10.9 10.6 100 Y9 28 93.8 10.2 Stems Per Plant (#) Atlantic Ctrl 28 3.3 0.9439 0.5 1 6 Y9 28 3.3 0.7 Plant Vigor (1-5 Scale) Atlantic Ctrl 28 4.1 0.8785 0.9 1.3 5 Y9 28 4.1 1.1 Plant Height (cm) Atlantic Ctrl 28 59.5 0.8858 15.6 16.4 108.7 Y9 28 59.2 16.5 Vine Desiccation (%) Atlantic Ctrl 28 42.5 0.1516 28.7 0 100 Y9 28 50.5 25.4 Tuber Evaluation Total Yield (cwt/a) Atlantic Ctrl 28 566.5 0.393 201.3 89.2 1410.6 Y9 28 535.7 198.0 US#1 Yield (cwt/a) Atlantic Ctrl 28 512.5 0.1676 202.4 118.9 693.5 Y9 28 467.5 206.3 Tubers Per Plant (#) Atlantic Ctrl 28 11.6 0.7709 4.0 3.1 19.5 Y9 28 11.8 3.6 A (%) Atlantic Ctrl 28 67.9 0.8448 12.3 28 83.3 Y9 28 67.1 7.9 B (%) Atlantic Ctrl 28 8.6 0.0564 8.3 2 70.5 Y9 28 11.2 8.8 Oversized (%) Atlantic Ctrl 28 17.8 0.3732 16.0 0 45.7 Y9 28 14.7 11.3 Pick-outs (%) Atlantic Ctrl 28 2.9 0.1471 3.8 0 17.3 Y9 28 4.9 5.5 Specific Gravity Atlantic Ctrl 28 1.089 0.0003 0.0086 0.835 1.171 Y9 28 1.092 0.0092 Total Internal Defects (%) 28 3.2 0.7891 1.7 0 93.8 28 3.4 1.6

The phenotypic performance, tuber evaluation, and ecological interactions studies did not indicate any meaningful differences between Y9 and the Atlantic control. There were no statistical differences detected for any of the phenotypic characteristics. For the tuber assessment, specific gravity was higher for Y9 compared to the control, but within the range of values seen in conventional potatoes. This change would not alter the environmental impact of Y9 which is the same as conventional potatoes. The lack of differences for insect, disease, and abiotic stressors as well as arthropod abundance supports a conclusion that the ecological interactions of Y9 are the same as conventional potatoes.

Example 10A: Potato Cultivar Y9 Late Blight Efficacy 2013 Experiments

The purpose of this study was to evaluate the field efficacy of potato event Y9 against foliar late blight (Phytophthora infestans).

Field trials were conducted at three sites during 2013. Plots were inoculated with the US-8, US-22, and/or US-23 strains of late blight. The degree of foliar infection was rated throughout the season.

A significant reduction in late blight foliar infection was observed in Y9 compared to their non-transformed parental controls, demonstrating efficacy of the late blight resistance trait against the strains of P. infestans tested.

Example 10B: Potato Cultivar Y9 Late Blight Efficacy 2014 Experiments

The purpose of this study was to evaluate the field efficacy of potato event Y9 against foliar late blight (Phytophthora infestans).

Field trials were conducted at two sites during 2014. Plots were inoculated with the US-23 strain of late blight. The degree of foliar infection was rated throughout the season.

A significant reduction in late blight foliar infection was observed in Y9 compared to their non-transformed parental controls, demonstrating efficacy of the late blight resistance trait against the strain of P. infestans tested.

INCORPORATION BY REFERENCE

All references, articles, publications, patents, patent publications, and patent applications cited herein are incorporated by reference in their entireties for all purposes. However, mention of any reference, article, publication, patent, patent publication, and patent application cited herein is not, and should not be taken as an acknowledgment or any form of suggestion that they constitute valid prior art or form part of the common general knowledge in any country in the world.

It should be understood that the above description is only representative of illustrative embodiments and examples. For the convenience of the reader, the above description has focused on a limited number of representative examples of all possible embodiments, examples that teach the principles of the disclosure. The description has not attempted to exhaustively enumerate all possible variations or even combinations of those variations described. That alternate embodiments may not have been presented for a specific portion of the disclosure, or that further undescribed alternate embodiments may be available for a portion, is not to be considered a disclaimer of those alternate embodiments. One of ordinary skill will appreciate that many of those undescribed embodiments, involve differences in technology and materials rather than differences in the application of the principles of the disclosure. Accordingly, the disclosure is not intended to be limited to less than the scope set forth in the following claims and equivalents.

REFERENCES

-   Chawla, R., Shakya, R., and Rommens, C. M. (2012). Tuber-Specific     Silencing of Asparagine synthetase-1 Reduces the Acrylamide-Forming     Potential of Potatoes Grown in the Field without Affecting Tuber     Shape and Yield. Plant Biotechnology Journal 10, 913-924. -   Courvalin, P., Weisblum, B., and Davies, J. (1977).     Aminoglycoside-Modifying Enzyme of an Antibiotic-Producing Bacterium     Acts as a Determinant of Antibiotic Resistance in Escherichia coli.     Proceedings of the National Academy of Sciences 74, 999-1003. -   Garbarino, J. E., and Belknap, W. R. (1994). Isolation of a     Ubiquitin-Ribosomal Protein Gene (ubi3) from Potato and Expression     of Its Promoter in Transgenic Plants. Plant Molecular Biology 24,     119-127. -   Garbarino, J. E., Oosumi, T., and Belknap, W. R. (1995). Isolation     of a Polyubiquitin Promoter and Its Expression in Transgenic Potato     Plants. Plant Physiology 109, 1371-1378. -   Simpson, J., Timko, M. P., Cashmore, A. R., Schell, J., Van Montagu,     M., and Herrera-Estrella, L. (1985). Light-Inducible and     Tissue-Specific Expression of a Chimaeric Gene under Control of the     5′-Flanking Sequence of a Pea Chlorophyll A/b-Binding Protein Gene.     The EMBO Journal 4, 2723-2729. -   Smigocki, A. C., and Owens, L. D. (1988). Cytokinin Gene Fused with     a Strong Promoter Enhances Shoot Organogenesis and Zeatin Levels in     Transformed Plant Cells. Proceedings of the National Academy of     Sciences 85, 5131-5135. -   VanHaaren, M. J. J., Sedee, N. J. A., de Boer, H. A.,     Schilperoort, R. A., and Hooykaas, P. J. J. (1989). Mutational     Analysis of the Conserved Domains of a T-Region Border Repeat of     Agrobacterium tumefaciens. Plant Molecular Biology 13, 523-531.

DEPOSIT INFORMATION

A tuber deposit of the J. R. Simplot Company proprietary POTATO CULTIVAR Y9 disclosed above and recited in the appended claims has been made with the American Type Culture Collection (ATCC), 10801 University Boulevard, Manassas, Va. 20110. The date of deposit was Jun. 17, 2015. The deposit of 50 vials of microtubers was taken from the same deposit maintained by J.R. Simplot Company since prior to the filing date of this application. All restrictions will be irrevocably removed upon granting of a patent, and the deposit is intended to meet all of the requirements of 37 C.F.R. §§ 1.801-1.809. The ATCC Accession Number is PTA-122247. The deposit will be maintained in the depository for a period of thirty years, or five years after the last request, or for the enforceable life of the patent, whichever is longer, and will be replaced as necessary during that period. 

What is claimed is:
 1. A potato tuber, or a part of a tuber, of potato cultivar Y9, wherein a representative sample of said tuber was deposited under ATCC Accession No. PTA-122247.
 2. A potato plant, or a part thereof, produced by growing the tuber, or a part of the tuber, of claim
 1. 3. A potato plant having all of the physiological and morphological characteristics of the plant of claim 2, and comprising the insert region of pSIM1278 that is present in cultivar Y9 which contains inverted repeats of potato DNA effective for inhibition of expression of the endogenous asparagine synthetase-1 gene and the endogenous polyphenol oxidase-5 gene in addition to inverted repeats of the endogenous potato promoters for the phosphorylase-L and dikinase R1 genes and further comprising the insert region of pSIM1678 that is present in Y9 which contains the potato late blight resistance gene Rpi-vnt1 and inverted repeats of potato DNA effective for inhibition of expression of the endogenous vacuolar invertase gene VInv.
 4. A tissue culture of cells produced from the plant of claim 2, wherein said cells of the tissue culture are produced from a plant part selected from the group consisting of leaf, pollen, embryo, cotyledon, hypocotyl, meristematic cell, root, root tip, pistil, anther, flowers, stem and tuber, and wherein said tissue cultured cells comprise the insert region of pSIM1278 that is present in cultivar Y9 which contains inverted repeats of potato DNA effective for inhibition of expression of the endogenous asparagine synthetase-1 gene and the endogenous polyphenol oxidase-5 gene in addition to inverted repeats of the endogenous potato promoters for the phosphorylase-L and dikinase R1 genes and further comprising the insert region of pSIM1678 that is present in Y9 which contains the potato late blight resistance gene Rpi-vnt1 and inverted repeats of potato DNA effective for inhibition of expression of the endogenous vacuolar invertase gene VInv.
 5. A potato plant regenerated from the tissue culture of claim 4, wherein said plant has all of the physiological and morphological characteristics of potato cultivar Y9.
 6. A potato seed produced by growing the potato tuber, or a part of the tuber, of claim 1, wherein said seed comprises the insert region of pSIM1278 that is present in cultivar Y9 which contains inverted repeats of potato DNA effective for inhibition of expression of the endogenous asparagine synthetase-1 gene and the endogenous polyphenol oxidase-5 gene in addition to inverted repeats of the endogenous potato promoters for the phosphorylase-L and dikinase R1 genes and further comprising the insert region of pSIM1678 that is present in Y9 which contains the potato late blight resistance gene Rpi-vnt1 and inverted repeats of potato DNA effective for inhibition of expression of the endogenous vacuolar invertase gene VInv.
 7. A potato plant, or a part thereof, produced by growing the seed of claim
 6. 8. A potato plant regenerated from tissue culture of the potato plant of claim 7, wherein said regenerated plant comprises the insert region of pSIM1278 that is present in cultivar Y9 which contains inverted repeats of potato DNA effective for inhibition of expression of the endogenous asparagine synthetase-1 gene and the endogenous polyphenol oxidase-5 gene in addition to inverted repeats of the endogenous potato promoters for the phosphorylase-L and dikinase R1 genes and further comprising the insert region of pSIM1678 that is present in Y9 which contains the potato late blight resistance gene Rpi-vnt1 and inverted repeats of potato DNA effective for inhibition of expression of the endogenous vacuolar invertase gene VInv.
 9. A method for producing a potato seed, said method comprising crossing two potato plants and harvesting the resultant potato seed, wherein at least one potato plant is the potato plant of claim
 2. 10. A method for producing a potato seed, said method comprising crossing two potato plants and harvesting the resultant potato seed, wherein at least one potato plant is the potato plant of claim
 7. 11. A potato seed produced by the method of claim 10, wherein said seed comprises the insert region of pSIM1278 that is present in cultivar Y9 which contains inverted repeats of potato DNA effective for inhibition of expression of the endogenous asparagine synthetase-1 gene and the endogenous polyphenol oxidase-5 gene in addition to inverted repeats of the endogenous potato promoters for the phosphorylase-L and dikinase R1 genes and further comprising the insert region of pSIM1678 that is present in Y9 which contains the potato late blight resistance gene Rpi-vnt1 and inverted repeats of potato DNA effective for inhibition of expression of the endogenous vacuolar invertase gene VInv.
 12. A potato plant, or a part thereof, produced by growing said potato seed of claim
 11. 13. A potato seed produced from the plant of claim 12, wherein said seed comprises the insert region of pSIM1278 that is present in cultivar Y9 which contains inverted repeats of potato DNA effective for inhibition of expression of the endogenous asparagine synthetase-1 gene and the endogenous polyphenol oxidase-5 gene in addition to inverted repeats of the endogenous potato promoters for the phosphorylase-L and dikinase R1 genes and further comprising the insert region of pSIM1678 that is present in Y9 which contains the potato late blight resistance gene Rpi-vnt1 and inverted repeats of potato DNA effective for inhibition of expression of the endogenous vacuolar invertase gene VInv.
 14. The method of claim 9, wherein one of said potato plants is potato cultivar Y9 and the second potato plant is transgenic.
 15. A method of producing a potato seed, said method comprising crossing two potato plants and harvesting the resultant potato seed, wherein one of said potato plants is the potato plant of claim 7 and the second potato plant is transgenic.
 16. A potato plant, or a part thereof, produced by growing the seed produced by the method of claim 14, wherein said plant comprises the insert region of pSIM1278 that is present in cultivar Y9 which contains inverted repeats of potato DNA effective for inhibition of expression of the endogenous asparagine synthetase-1 gene and the endogenous polyphenol oxidase-5 gene in addition to inverted repeats of the endogenous potato promoters for the phosphorylase-L and dikinase R1 genes and further comprising the insert region of pSIM1678 that is present in Y9 which contains the potato late blight resistance gene Rpi-vnt1 and inverted repeats of potato DNA effective for inhibition of expression of the endogenous vacuolar invertase gene VInv.
 17. A method of introducing a desired trait into potato cultivar Y9, wherein the method comprises: (a) crossing a Y9 plant, wherein a representative sample of tubers was deposited under ATCC Accession No. PTA-122247, with a plant of another potato cultivar that comprises a desired trait to produce progeny plants, wherein the desired trait is selected from the group consisting of male sterility, herbicide resistance, insect resistance, modified fatty acid metabolism, modified carbohydrate metabolism and resistance to bacterial disease, fungal disease or viral disease; (b) selecting one or more progeny plants that have the desired trait; (c) backcrossing the selected progeny plants with Y9 plants to produce backcross progeny plants; (d) selecting for backcross progeny plants that have the desired trait; and (e) repeating steps (c) and (d) two or more times in succession to produce selected third or higher backcross progeny plants that comprise the desired trait.
 18. A potato plant produced by the method of claim 17, wherein the plant has the desired trait and comprises the insert region of pSIM1278 that is present in cultivar Y9 which contains inverted repeats of potato DNA effective for inhibition of expression of the endogenous asparagine synthetase-1 gene and the endogenous polyphenol oxidase-5 gene in addition to inverted repeats of the endogenous potato promoters for the phosphorylase-L and dikinase R1 genes and further comprising the insert region of pSIM1678 that is present in Y9 which contains the potato late blight resistance gene Rpi-vnt1 and inverted repeats of potato DNA effective for inhibition of expression of the endogenous vacuolar invertase gene VInv.
 19. The potato plant of claim 18, wherein the desired trait is herbicide resistance and the resistance is conferred to an herbicide selected from the group consisting of imidazolinone, sulfonylurea, glyphosate, glufosinate, L-phosphinothricin, triazine and benzonitrile.
 20. The potato plant of claim 18, wherein the desired trait is insect resistance and the insect resistance is conferred by a transgene encoding a Bacillus thuringiensis endotoxin.
 21. The potato plant of claim 18, wherein the desired trait is modified fatty acid metabolism or modified carbohydrate metabolism and said desired trait is conferred by a nucleic acid encoding a protein selected from the group consisting of fructosyltransferase, levansucrase, α-amylase, invertase and starch branching enzyme or DNA encoding an antisense of stearyl-ACP desaturase.
 22. A method of producing a commodity plant product, comprising obtaining the plant of claim 2, or a part thereof, and producing the commodity plant product from said plant or plant part thereof, wherein said commodity plant product is selected from the group consisting of: fresh whole potatoes, French fries, potato chips, dehydrated potato material, potato flakes and potato granules.
 23. The commodity plant product produced by the method of claim 22, wherein said product comprises the insert region of pSIM1278 that is present in cultivar Y9 which contains inverted repeats of potato DNA effective for inhibition of expression of the endogenous asparagine synthetase-1 gene and the endogenous polyphenol oxidase-5 gene in addition to inverted repeats of the endogenous potato promoters for the phosphorylase-L and dikinase R1 genes and further comprising the insert region of pSIM1678 that is present in Y9 which contains the potato late blight resistance gene Rpi-vnt1 and inverted repeats of potato DNA effective for inhibition of expression of the endogenous vacuolar invertase gene VInv.
 24. A food product made from the potato tuber of claim
 1. 25. A food product made from the potato tuber of claim 1, wherein the food product is a sliced potato tuber food product.
 26. A food product made from the potato tuber of claim 1, wherein the food product is a French fry or chip.
 27. A heat-processed tuber product obtained from the potato tuber of claim
 1. 28. A heat-processed tuber product obtained from the potato tuber of claim 1, wherein the heat processed tuber product is selected from the group consisting of: a French fry, a chip, and a baked potato.
 29. A heat-processed tuber product obtained from the potato tuber of claim 1, wherein the heat processed tuber product is selected from the group consisting of: a French fry, a chip, and a baked potato, wherein the heat-processed tuber product has a concentration of acrylamide that is at least 50% lower, 60% lower, 70% lower, 80% lower, 85% lower, or more, than the concentration of acrylamide of a control heat-processed tuber product that is obtained from a control potato plant that does not comprise the insert region of pSIM1278 and pSIM1678 that is present in cultivar Y9. 